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Abstract

Background

Although Ixodes spp. are the most common ticks in North-Western Europe, recent reports indicated
an expanding geographical distribution of Dermacentor reticulatus in Western Europe. Recently, the establishment of a D. reticulatus population in Belgium was described. D. reticulatus is an important vector of canine and equine babesiosis and can transmit several Rickettsia species, Coxiella burnetii and tick-borne encephalitis virus (TBEV), whilst Ixodes spp. are vectors of pathogens causing babesiosis, borreliosis, anaplasmosis, rickettsiosis
and TBEV.

Methods

A survey was conducted in 2008-2009 to investigate the presence of different tick
species and associated pathogens on dogs and cats in Belgium. Ticks were collected
from dogs and cats in 75 veterinary practices, selected by stratified randomization.
All collected ticks were morphologically determined and analysed for the presence
of Babesia spp., Borrelia spp., Anaplasma phagocytophilum and Rickettsia DNA.

Results

In total 2373 ticks were collected from 647 dogs and 506 cats. Ixodes ricinus (76.4%) and I. hexagonus (22.6%) were the predominant species. Rhipicephalus sanguineus (0.3%) and D. reticulatus (0.8%) were found in low numbers on dogs only. All dogs infested with R. sanguineus had a recent travel history, but D. reticulatus were collected from a dog without a history of travelling abroad. Of the collected
Ixodes ticks, 19.5% were positive for A. phagocytophilum and 10.1% for Borrelia spp. (B. afzelii, B. garinii, B. burgdorferi s.s., B. lusitaniae, B. valaisiana and B. spielmanii). Rickettsia helvetica was found in 14.1% of Ixodes ticks. All Dermacentor ticks were negative for all the investigated pathogens, but one R. sanguineus tick was positive for Rickettsia massiliae.

Conclusion

D. reticulatus was confirmed to be present as an indigenous parasite in Belgium. B. lusitaniae and R. helvetica were detected in ticks in Belgium for the first time.

Keywords:

Background

The most common tick in North-Western Europe is the sheep or castor bean tick, Ixodes ricinus. This tick species is also widely distributed in Belgium [1]. Ixodes ticks are vectors of a broad range of pathogens of medical and veterinary importance,
such as Babesia spp., Borrelia spp., Anaplasma phagocytophilum, Rickettsia spp., Bartonella spp. and tick-borne encephalitis virus (TBEV). The brown dog tick, Rhipicephalus sanguineus and the European meadow tick, Dermacentor reticulatus are occasionally introduced into Northern Europe with imported dogs or by dogs travelling
from endemic areas. R. sanguineus is a vector of, among others, Babesia vogeli, Ehrlichia canis, Hepatozoon canis, Rickettsia conorii and Cercopithifilaria spp. D. reticulatus is an important vector of canine and equine babesiosis and can transmit Rickettsia spp., Francisella tularensis, Coxiella burnetii and TBEV. Until recently, the French-Belgian border was considered to be the northern
boundary of the distribution of D. reticulatus in Western Europe [2]. However, recent reports indicated that the habitat of D. reticulatus is expanding in North-Western Europe, with several foci now present in The Netherlands
[3] and in Germany [4]. The occurrence of autochthonous cases of canine babesiosis in Belgium during the
last two decades [5] suggests that this tick species could also be indigenous in this country. Low numbers
of D. reticulatus were previously found on dogs in Belgium (Losson et al., personal communications), but it was not clear whether these ticks belonged to
indigenous tick populations or were imported after travelling abroad and the presence
of tick-borne pathogens in these ticks was not investigated. Therefore, a new survey
was conducted in 2008-2009 to investigate the presence of different tick species collected
from dogs and cats in Belgium and their associated pathogens. Dogs and cats were chosen,
because several tick-borne diseases are of clinical importance in dogs and/or cats
(e.g. babesiosis and ehrlichiosis) and because dogs and cats live in the close vicinity
of their owners and can act as direct sentinels for infection of humans [6]. The approach of gathering data on the distribution of (zoonotic) vector-borne diseases
through a veterinary survey is consistent with the ‘One Health’ concept [7,8]. Based on the recurrent collection of D. reticulatus ticks from a dog in this study, the presence of an indigenous D. reticulatus population in Belgium was confirmed by flagging at the study site [9].

Methods

Tick collection

A nationwide survey was performed in Belgium from April 2008 to April 2009. For each
of the 25 veterinary districts, 3 companion animal practices were selected by stratified
randomization (Figure 1). Ticks from cats and dogs, randomly submitted to seventy-five veterinary practices,
were collected and preserved in 80% alcohol. For each animal enrolled in the study,
information was recorded by the veterinarian about location, date of collection, animal
description (dog/cat, age, sex, breed), the location on the host where the tick was
found, whether the animal had travelled outside Belgium during the previous 2 weeks
and whether the animal showed clinical signs that could be associated with a tick-borne
disease, such as fever, apathy, anorexia, arthritis, anaemia or meningitis. The ticks
were identified to species level, with stage and sex recorded, using a standard morphological
key [10]. When D. reticulatus ticks were found on an animal without history of travel to a country known to be
endemic for this tick species, the veterinarian or the owner was contacted for more
information regarding the area in Belgium where the animal might have acquired the
tick. These areas were subsequently surveyed for the presence of D. reticulatus by flagging the vegetation with a flannel cloth [9].

Figure 1.Distribution of selected veterinary practices and presence of an indigenous Dermacentor reticulatus population (red dot) in Belgium.

DNA extraction, PCR amplification and sequencing

One tick (nymph or adult) per animal was selected for DNA analyses, but when several
tick species were present on a given animal, one tick of each species was randomly
selected for further analysis. Tick DNA extraction was performed using a protocol
with proteinase K [11]. In order to detect false negative results due to PCR inhibition and to validate
the efficiency of the DNA extraction, a PCR targeting a 325 bp DNA fragment corresponding
to the tick 16S rRNA gene was included, using 16S + 1 and 16S-2 primers [12].

The presence of Babesia spp., B. burgdorferi s.l., A. phagocytophilum and Rickettsia spp. DNA in tick DNA extracts was tested by PCR using specific primers for each pathogen.
The primer sets and PCR conditions used for the different pathogens are listed in
Table 1. A Babesia spp. specific PCR was based on the amplification of a 411-452 bp fragment of the
multicopy 18S rRNA gene [13]. For the detection of A. phagocytophilum, a real-time PCR was performed according to [14], to amplify a 77-bp segment at the conserved amino-terminal coding region of the
msp2 gene. All samples, a negative and a positive control were run in duplicate, and samples
with a Cp (crossing point of the amplification curve) above 35 cycles were considered negative.
For Borrelia spp. a specific nested PCR was developed targeting the flagellin gene, resulting
in a 193 bp fragment. The first reaction was carried out in a 25 μl volume containing
0.2 μM of each dNTP, 0.2 μM of each primer, 1.5 mM MgCl2, 5 μl of 5× buffer, 0.625 U of Taq and 2.5 μl of the DNA extract. The second reaction
was conducted on 2.5 μl of a 1/10 dilution of the first PCR product and contained
in 25 μl 0.2 μM of each dNTP, 0.2 μM of each primer, 1.5 mM MgCl2, 5 μl of 5× buffer and 0.625 U of Taq. Plasmids containing genomic DNA of Borrelia spp. were kindly provided by F. Jongejan (Utrecht University, The Netherlands) and
H. Sprong (RIVM, The Netherlands). DNA from Rickettsia spp. was detected using the rapidSTRIPE Rickettsia Assay (Analytik Jena, Jena, Germany),
following the manufacturer’s instructions. Positive samples were confirmed by PCR,
targeting the citrate synthase gene (gltA) with the Rsfg877/Rsfg1258 primers, which results in amplification of a 380 bp fragment
[15].

Tick DNA samples positive for Babesia spp. were sequenced as described by [13]. Samples that were positive for A. phagocytophilum were sent to GATC Biotech AB (Konstanz, Germany) for sequence analysis. Borrelia and Rickettsia PCR products were purified using the Qiaquick® purification kit (Qiagen) and fully
sequenced in both directions using the Big Dye Terminator V3.1 Cycle sequencing Kit
(Applied Biosystems). Sequencing reactions were analysed on a 3100 Genetic Analyzer
(Applied Biosystems) and assembled with Seqman II (DNASTAR, Madison WI, USA). Sequences
were compared with reference sequences by BLAST-analysis against the NCBI database.

Statistical analysis

Pathogen infection rates and 95% confidence intervals were calculated for each pathogen.

The χ2-test was used to compare infection rates of pathogens between I. ricinus and I. hexagonus ticks, to compare infection rates for the different pathogens in ticks collected
from dogs and cats with or without clinical signs indicative for tick-borne disease
and to compare tick infection rates between northern Belgium (Flanders) and southern
Belgium (Wallonia). A p-value of 0.05 was considered statistically significant.

Results

Tick identification

A total of 2373 ticks were collected from 647 dogs and 506 cats. The number of ticks
per animal ranged from 1 to 34, but most submissions (70%) only contained a single
tick. Most of the collected ticks were Ixodes spp. In cats, I. ricinus (80.1% of infested cats, 95% CI: 77.0–83.9) and I. hexagonus (23.4%, 95% CI: 19.9–27.3) were the only tick species found. The most frequently
found tick species in dogs was also I. ricinus (82.1% of infested dogs, 95% CI: 78.9–84.9), followed by I. hexagonus (18.9%, 95% CI: 15.9–22.2). Ticks were submitted throughout the year. Most I. ricinus ticks were collected during springtime, with a peak in May 2008 (843 ticks,). Most
I. hexagonus were also recorded during this period, but a second, smaller peak occurred in October
2008. The majority of the ticks that were collected from dogs, were located on the
head (42.7%), the neck (21.7%) and the thorax/abdomen (22.6%). In cats, most ticks
were recovered from the head (40.9%) and the neck (41.6%). The majority of the recovered
ticks were adults (89.2%), only 8.3% were nymphs and 2.6% larvae.

R. sanguineus and D. reticulatus were only found on 4 and 6 dogs, respectively. All dogs infested with R. sanguineus and 5 out of 6 dogs infested with D. reticulatus had a recent travel history (to France, Italy or an unspecified country), but D. reticulatus ticks were repeatedly collected from one dog without a history of travelling abroad.
The presence of an indigenous population of D. reticulatus was confirmed by flagging the area where this dog was regularly taken for a walk
(Beveren-Waas, Flanders, 51°12’02”N, 4°14’15”E) (Figure 1) [9].

All Dermacentor ticks were negative for all the investigated pathogens, but one R. sanguineus tick was found positive for Rickettsia massiliae (EMBL accession number HF930724).

Most of the animals were healthy at the time of tick collection. Nevertheless, one
cat showed swelling and pain at the site where a Borrelia- positive tick was attached. One cat and five dogs that were infested with ticks that
contained A. phagocytophilum DNA, showed either local swelling or inflammation at the site of tick collection
(n = 4, one co-infection with Borrelia), lameness (n = 1) or weight loss (n = 1). One dog with a Rickettsia-positive tick had arthritis. However, 13 cats and 16 dogs also showed clinical signs
that have been associated with tick-borne diseases, such as acute malaise (apathy,
fever, anorexia), lameness, lymphadenopathy, glomerulonephritis or neurological signs,
while collected ticks were negative for all investigated pathogens. There was no significant
difference in the detection rates of B. burgdorferi s.l. (χ2 =2.31, d.f. = 1, P = 0.13), A. phagocytophilum (χ2 =0.13, d.f. = 1, P = 0.72) or R. helvetica (χ2 =3.53, d.f. = 1, P = 0.60) between ticks collected from animals with or without
clinical signs.

Discussion

In this study I. ricinus was the predominant tick species infesting companion animals, followed by the hedgehog
tick, I. hexagonus. This is in analogy with other studies in North-Western Europe. Similar results were
reported from The Netherlands [3], Germany [16] and the UK [17,18]. In the UK and Ireland, the fox tick I. canisuga was also frequently recovered from dogs [17,18]. Ogden et al. [17] found I. ricinus on a significantly higher proportion of dogs than cats, while I. hexagonus was more frequently found on cats. They suggested that differences in behaviour between
dogs and cats could affect their likelihood of encountering both Ixodes species. This hypothesis was not supported by our data, with similar proportions
of dogs and cats carrying I. ricinus and I. hexagonus. Equal proportions of both Ixodes species were also recovered from dogs and cats in Germany [16] and The Netherlands [3]. The recovered Ixodes ticks were mainly adults, as was also observed in other studies in dogs and cats
[16,18,19]. Although it cannot be excluded that some nymphs and larvae were overlooked in the
clinical inspections, adult Ixodes ticks are known to attach preferably to large or medium-sized mammals, including
dogs and cats [20].

Generally, nymphs and adults of I. ricinus show a marked seasonal variability in their questing activity, with a first peak
in late spring and early summer and a second peak in autumn [21,22]. This seasonal pattern was also observed in the number of ticks recovered from dogs
by [18] and [19]. In this study, we observed an obvious spring peak, but only low numbers of I. ricinus were submitted in autumn. Although participation rates of the veterinarians may have
introduced a bias, tick questing activity may be variable from year to year and a
single spring or summer peak has previously been observed for questing I. ricinus nymphs [23] and for adult I. ricinus on dogs [16]. Most I. hexagonus were also recovered in the spring in our study, but a second, smaller peak occurred
in October. Only limited published information is available on the seasonal abundance
of I. hexagonus ticks, but seasonal fluctuations in numbers of I. hexagonus collected from dogs and hedgehogs are generally weaker compared to I. ricinus[16,24].

The majority of infected ticks were found in Northern Belgium (Flanders). The north-eastern
part of Belgium (the Campine) is known to be heavily infested with Ixodes and has a relatively high incidence of Lyme borreliosis [25]. Although the south-eastern part of Belgium has a lot of forest and would also be
expected to have a lot of good Ixodes habitats, the number of ticks positive for tick-borne diseases from that area was
lower in our study. The reason for this remains unclear.

There was no significant difference between I. ricinus and I. hexagonus in the proportion of ticks that contained DNA from B. burgdorferi s.l., A. phagocytophilum or R. helvetica. Although both I. ricinus and I. hexagonus can be vectors of Borrelia spp. and A. phagocytophilum[26,27], I. ricinus is considered to be the principal vector of these pathogens [27,28]. As a nest dwelling species, I. hexagonus will have little direct contact with humans. Nevertheless, I. hexagonus could be a vector for the transmission of Borrelia spp. and A. phagocytophilum to hedgehogs, and then via co-infections with I. ricinus indirectly to humans [24,27].

The percentage of ticks positive for Borrelia spp. was within the range of infection rates (2.3-22%) in ticks collected from dogs
in other European countries [3,16,29-31]. Similar infection rates were also reported in questing I. ricinus in Belgium (12-23%) [32,33]. Within the B. burgdorferi sensu lato group, B. afzelii and B. garinii are the most common species in The Netherlands, Belgium and northern France, while
B. burgdorferi s.s. is less common in this region [34]. B. valaisiana has also been repeatedly found in The Netherlands (e.g. 3, 29). Together with other recent studies in Belgium and Luxembourg [33,35] our results show that besides B. valaisiana, B. spielmanii and B. lusitaniae are also present in Ixodes in the Benelux region. B. garinii, B. afzelii and B. burgdorferi s.s. are well known to be pathogenic for humans, but the pathogenic significance of the
other species is still unclear [36,37].

The majority of dogs and cats that are exposed to Borrelia infections remain clinically normal [20], which was also the case in this study. Most cases of canine Lyme borreliosis are
associated with B. burgdorferi s.s. Whilst B. burgdorferi s.s. is the only Borrelia species in the USA, prevalences of B. burgdorferi s.s. in Europe are much lower [34], as was also the case in this study. This may explain why lyme borreliosis is frequently
diagnosed in dogs in endemic regions in the USA, but less frequently in European dogs.

Although Borrelia can be transmitted from dogs to ticks, dogs are not considered as important reservoir hosts [20] and studies examining seropositivity in dogs, their owners and other local residents
found no correlation between dog ownership and infection risk [38-40]. Nevertheless, dogs and cats can be used as sentinels for lyme borreliosis. Serological
studies in the USA showed that exposure of dogs to B. burgdorferi mimics the geographical distribution of reports of Lyme borreliosis in humans [20] and the use of dog sera to detect and quantify the risk of Lyme borreliosis for humans
in a certain region is considered to be more sensitive than the use of incidence reports
of human clinical cases [40]. Seroprevalence has been found greater in dogs than in humans due to their greater
habitat exposure, lack of protective clothing and inability to check themselves from
ticks [38]. The use of dog sera also has the advantage over human serology that the seroprevalence
among dogs is more likely to reflect the actual environmental risk of Lyme borreliosis,
because of the short half-life of canine antibodies against B. burgdorferi[40]. However, serological studies are often limited by small sample sizes, and false
positive results are possible. Detection of Borrelia DNA in ticks collected from dogs and cats can be a valuable alternative [31].

The A. phagocytophilum infection rate in this study was much higher than previously reported point prevalences
in Ixodes ticks from dogs in The Netherlands and Poland (1.6-2.9%) [3,30]. Seroprevalences in dogs in Europe are also very variable, with prevalences from < 5%
to > 50% [41]. The percentage of seropositive dogs depends on the dog population sampled (e.g. healthy dogs vs. dogs with signs of tick-borne diseases) and geographical variation
in exposure to ticks and reservoir hosts. The high infection rate of A. phagocytophilum in ticks collected from dogs in this study is in contrast with the low incidence
of human granulocytic anaplasmosis (HGA) in Belgium (< 100/year) [25]. However, there is a discrepancy between the official (low) incidence rates [25] and the high number of HGA cases that are detected in specific surveys [42,43]. In a recent 10-year serological survey in patients with symptoms of tick-borne infections,
31% of the samples were positive, and 111 cases of HGA were confirmed [42]. These data suggest that Belgium is a hot spot for HGA and that many cases of HGA
probably remain undiagnosed [43].

Most dogs infected with A. phagocytophilum probably remain healthy [41]. The most common clinical signs in dogs that develop illness are lethargy, fever
and lameness. In the present study, no association was found between clinical signs
and the presence of A. phagocytophilum in ticks collected from these animals. Although identical 16S rRNA gene sequences
have been found in canine and human isolates of A. phagocytophilum in Europe [44,45], dogs are not thought to be important reservoirs for A. phagocytophilum, since bacteremia is of short duration in this species [46]. In Slovenia, no difference in seroprevalence was observed between people with or
without exposure to dogs [47].

Ixodes spp. can transmit several Rickettsia species belonging to the ‘spotted fever’ group, such as Rickettsia helvetica and R. monacensis. We found R. helvetica DNA in 14.1% of Ixodes ticks collected from dogs and cats in Belgium. In the Netherlands, 24.7% I. ricinus ticks and 0.8% I. hexagonus ticks collected from dogs, cats and a hedgehog were infected with R. helvetica[3]. In Switzerland, 40.9% and 17.6% of Ixodes ticks collected from cats and dogs, respectively, tested positive for R. helvetica with a gltA-specific TaqMan PCR system [48]. R. helvetica is a suspected pathogen in humans. Symptoms that have been associated with R. helvetica infections include fever, headache, arthralgia, myalgia and perimyocarditis [48]. The high prevalence of R. helvetica in Ixodes spp. and the high abundance of these tick species suggest that the likelihood of
transmission of R. helvetica to humans should be high [48]. However, despite a high infection rate (19%) of R. helvetica in ticks collected from humans in the Netherlands, no association between symptoms
and R. helvetica was found [49].

The clinical importance of R. helvetica in domestic animals is as yet uncertain and it is also unknown whether dogs and cats
can serve as a reservoir after infection. The fact that the estimated prevalence of
R. helvetica in ticks collected from dogs, cats and roe deer was higher than in ticks collected
from the vegetation [48,50] may indicate that large animals act as a reservoir for R. helvetica[48].

Next to I. ricinus and I. hexagonus, small numbers of R. sanguineus and D. reticulatus were collected from dogs. All submitted R. sanguineus ticks were considered to be imported, since they were all collected from dogs with
a history of travelling abroad, mostly to Southern Europe. One R. sanguineus tick contained DNA from R. massiliae. R. massiliae is suspected to be the main cause of Mediterranean spotted fever in Spain [51].

Although most submitted Dermacentor ticks were also from dogs with a travel history, D. reticulatus ticks were repeatedly sampled from one particular dog that had never been outside
Belgium. Flagging confirmed the presence of questing Dermacentor ticks in the area where the dog was walked daily [9]. This was the first finding of an indigenous population of D. reticulatus in Belgium. Further investigations have revealed the presence of at least 4 other
foci of D. reticulatus in Belgium (51, M. Madder, unpublished results).

Conclusions

Repeated collection of D. reticulatus from a dog without history of traveling led to the discovery of an indigenous population
of D. reticulatus in Belgium [9], confirming the geographical expansion of this tick species in North-western Europe.
High infection rates were found for Borrelia spp., A. phagocytophilum and R. helvetica in Ixodes ticks collected from dogs and cats in Belgium. B. lusitaniae and R. helvetica were detected in ticks in Belgium for the first time.

Abbreviations

TBEV: Tick-borne encephalitis virus.

Competing interests

This study was partially financed by Bayer Health Care, Animal Health Division. In
the last 5 years, EC has obtained funding from, lectured or consulted for the following
companies selling products to treat tick infestations in dogs and cats: Bayer Health
Care, Merial, Pfizer Animal Health.

Authors’ contributions

EC conceived of and designed the study, acquired funding, flagged for D. reticulatus in Beveren-Waas, conducted data analysis and drafted the manuscript. BL conceived
of and designed the study, acquired funding and helped drafting the manuscript. CC
and PH performed the real-time PCR analyses for A. phagocytophilum and flagged for D. reticulatus in Beveren-Waas. SC developed and performed the PCR analyses for Borrelia, carried out the rapid assay and PCRs for Rickettsia and conducted data analysis. A-CD participated in the design of the study and helped
drafting the manuscript. ADC contributed to the organisation of the study and identified
the ticks. MM helped drafting the manuscript and flagged for D. reticulatus in Beveren-Waas. CS helped in the design of the study. LL contributed to the organisation
of the study, identified the ticks, developed and performed the Babesia PCR, conducted data analysis and helped drafting the manuscript. All authors read
and approved the final manuscript.

Acknowledgements

Negative and positive control samples for A. phagocytophilum were kindly provided by T. Avsic-Zupanc, University of Ljubljana, Ljubljana, Slovenia.
Plasmids containing genomic DNA of Borrelia spp. were kindly provided by F. Jongejan (Utrecht University, The Netherlands) and
H. Sprong (RIVM, The Netherlands). N. Mencke (Bayer Health Care) is acknowledged for
reviewing the manuscript. The authors are grateful to the participating veterinarians
for submitting the ticks.